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一种获取组织化学染色标本的一致图像并进行定量分析的创新方法。

An innovative method for obtaining consistent images and quantification of histochemically stained specimens.

作者信息

Linden Michael A, Sedgewick Gerald J, Ericson Marna

机构信息

Department of Lab Medicine and Pathology, University of Minnesota, Minneapolis, Minnesota (MAL)

Imaging and Analysis, Saint Paul, Minnesota (GJS)

出版信息

J Histochem Cytochem. 2015 Apr;63(4):233-43. doi: 10.1369/0022155415568996. Epub 2015 Jan 9.

DOI:10.1369/0022155415568996
PMID:25575568
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4374058/
Abstract

Obtaining digital images of color brightfield microscopy is an important aspect of biomedical research and the clinical practice of diagnostic pathology. Although the field of digital pathology has had tremendous advances in whole-slide imaging systems, little effort has been directed toward standardizing color brightfield digital imaging to maintain image-to-image consistency and tonal linearity. Using a single camera and microscope to obtain digital images of three stains, we show that microscope and camera systems inherently produce image-to-image variation. Moreover, we demonstrate that post-processing with a widely used raster graphics editor software program does not completely correct for session-to-session inconsistency. We introduce a reliable method for creating consistent images with a hardware/software solution (ChromaCal™; Datacolor Inc., NJ) along with its features for creating color standardization, preserving linear tonal levels, providing automated white balancing and setting automated brightness to consistent levels. The resulting image consistency using this method will also streamline mean density and morphometry measurements, as images are easily segmented and single thresholds can be used. We suggest that this is a superior method for color brightfield imaging, which can be used for quantification and can be readily incorporated into workflows.

摘要

获取彩色明场显微镜的数字图像是生物医学研究和诊断病理学临床实践的一个重要方面。尽管数字病理学领域在全切片成像系统方面取得了巨大进展,但在标准化彩色明场数字成像以保持图像间一致性和色调线性方面所做的努力却很少。我们使用单一相机和显微镜获取三种染色剂的数字图像,结果表明显微镜和相机系统本身会产生图像间的差异。此外,我们证明使用广泛使用的光栅图形编辑软件程序进行后期处理并不能完全校正不同实验之间的不一致性。我们介绍了一种通过硬件/软件解决方案(ChromaCal™;Datacolor Inc., 新泽西州)创建一致图像的可靠方法,以及该方法在创建颜色标准化、保留线性色调水平、提供自动白平衡和将自动亮度设置为一致水平方面的功能。使用此方法产生的图像一致性还将简化平均密度和形态测量,因为图像易于分割且可使用单一阈值。我们认为这是一种用于彩色明场成像的优越方法,可用于定量分析并可轻松纳入工作流程。